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对表达和沉默的Xist等位基因5'区域进行体内紫外线和硫酸二甲酯足迹分析。

In vivo ultraviolet and dimethyl sulfate footprinting of the 5' region of the expressed and silent Xist alleles.

作者信息

Komura J i, Sheardown S A, Brockdorff N, Singer-Sam J, Riggs A D

机构信息

Biology Department, Beckman Research Institute of the City of Hope, Duarte, California 91010, USA.

出版信息

J Biol Chem. 1997 Apr 18;272(16):10975-80. doi: 10.1074/jbc.272.16.10975.

Abstract

The Xist (X inactive specific transcript) gene plays an essential role in X chromosome inactivation. To elucidate the mechanisms controlling Xist expression and X inactivation, we examined in vivo DNA-protein interactions in the Xist promoter region in a female mouse cell line (BMSL2), which has distinguishable Xist alleles. In vivo footprinting was accomplished by treatment of cells with dimethyl sulfate or ultraviolet light, followed by ligation-mediated polymerase chain reaction of purified DNA. The expressed allele on the inactive X chromosome and the silent allele on the active X chromosome were separated by the use of a restriction fragment length polymorphism prior to ligation-mediated polymerase chain reaction. The chromatin structure of the Xist promoter was found to be consistent with the activity state of the Xist gene. The silent allele (on the active X chromosome) showed no footprints, while the expressed allele (on the inactive X chromosome) showed footprints at a consensus sequence for a CCAAT box, two weak Sp1 sites, and a weak TATA box.

摘要

Xist(X染色体失活特异性转录本)基因在X染色体失活过程中起着至关重要的作用。为了阐明控制Xist表达和X染色体失活的机制,我们在具有可区分Xist等位基因的雌性小鼠细胞系(BMSL2)中研究了Xist启动子区域的体内DNA-蛋白质相互作用。通过用硫酸二甲酯或紫外线处理细胞,然后对纯化的DNA进行连接介导的聚合酶链反应来完成体内足迹分析。在连接介导的聚合酶链反应之前,利用限制性片段长度多态性分离失活X染色体上的表达等位基因和活性X染色体上的沉默等位基因。发现Xist启动子的染色质结构与Xist基因的活性状态一致。沉默等位基因(在活性X染色体上)未显示足迹,而表达等位基因(在失活X染色体上)在CCAAT框、两个弱Sp1位点和一个弱TATA框的共有序列处显示足迹。

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